This invention provides for a method for treatment of corneal and dermal wounds by administering bismuth compounds in topical dosage forms. Bismuth compounds cause stimulation of release of growth factors in damaged tissue to promote regeneration of epithelial cells and hence accelerate wound healing. These bismuth compounds also have good antimicrobial activity against several anaerobic bacteria involved in diaper rash exacerbation.

8. A method of stimulating cellular production or release of growth factors, comprising the step of administering to corneal cells in an eye in need thereof a preparation comprising a bismuth compound in a topical dosage form to stimulate said cellular production or release of growth factors.

10. The method of claim 8, wherein said topical dosage form is selected from the group consisting of ointments, gels, creams, solutions, suspensions, emulsions, dressings, erodible and non-erodible inserts, and aerosols.

11. The method of claim 8, wherein said topical dosage form provides sustained release of bismuth compound in the eye to promote wound healing.

12. The method of claim 8, wherein said topical dosage form is a polymeric insert from which the bismuth compound is released over a 30-minute to 72-hour period.

13. The method of claim 8, wherein said topical dosage form is a soft contact lens impregnated with a bismuth compound to provide release over a 30-minute to 72-hour period.

This application is a continuation of application Ser. No. 09/253,559, filed Feb. 19, 1999, abandoned, which is a continuation of U.S. application Ser. No. 08/918,322 filed Aug. 26, 1997 and now abandoned which is a continuation-in-part of co-pending U.S. application Ser. No. 08/518,971, filed Aug. 24, 1995, now abandoned, which in turn is a continuation-in-part of U.S. application Ser. No. 08/385,060, filed Feb. 7, 1995, now abandoned, which in turn claims priority under 35 U.S.C. §119 to Japanese Application No. 6-93518, filed May 2, 1994. All of the above-identified applications are expressly incorporated herein by reference.

BACKGROUND OF THE INVENTION

Until recently, excessive gastric acidity and mental stress were thought to be major pathophysiological reasons for occurrence of peptic ulcers. In the early 1980, Marshall and Warren (Warren, Lancet, 1:1273-1275, 1983 and Marshall et al., Lancet, 2:1311-1315, 1984) first reported an unidentified curved bacilli in the stomach of patients with gastritis and peptic ulcers. These bacilli, which later were identified as a gram negative spiral bacterium and named Helicobacter pylori (Goodwin et al., Int. J. Syst. Bacteriol. 32:397-405, 1989), have been demonstrated to be associated with gastritis and peptic ulcers (Buck et al., J. Infect. Dis. 153:664-669, 1986 and Graham, Gastroenterology 26:615-625, 1989), and are thought to be transmitted by person-to-person contact. H. Pylori in the dental plaque (Nguyen et al., Journal of Clinical Microbiology 31(4):783-787, 1993; Desai et al., Scandinavian Journal of Gastroenterology 26:1205-1208, 1991; and Lambert et al., Lancet 341(8850):957, 1993), and have also shown that standard oral hygiene practice does not help reduce H. Pylori presence in the oral cavity (Nguyen et al., Journal of Clinical Microbiology 31(4):783-787, 1993). As a result of these recent discoveries associating bacterial infection in the causation of peptic ulcer disease, questions regarding the previously established paradigms of ulcer treatment and healing processes have been raised.

H2 receptor blockers which suppress acid secretion, such as cimetidine (Tagamet®) and ranitidine (Zantac®), have been used to treat and heal duodenal ulcers (Jones et al., Gut. 2:1120-1127, 1987; McIsaac et al., Aliment. Pharmacol. Therap. 1:369-381, 1987; and Boyed et al., Amsterdam:Excerpta Medica, 14-42, 1984). Recently, however, a number of clinical investigations have demonstrated that 70-80% of healed duodenal ulcers reoccur within the next year (Goodwin et al., Int. J. Syst. Bacteriol 22:397407, 1989), and that these drugs do not reverse the tendency for ulcers to form (Wormsley, British Medical Journal 293:1501, 1986; Gudman et al., British Medical Journal i:1095-1097, 1978; and Bardhan et al., British Medical Journal 29:621-623, 1982).

In addition to its bacteriocidal activity, CBS has been demonstrated to enhance mucus glycoprotein secretion, strengthen viscoelastic gel properties of mucus, cause increased concentration of epithelial growth factor (EGF) in ulcer tissue, and stimulate prostaglandin synthesis in the gastric antral mucosa (Lee, Scandinavian Journal of Gastroenterology 26(Supplement 185):1-6, 1991). These gastroprotective properties of CBS may contribute to the initial healing of duodenal ulcers and the observed lower rates of relapse by returning the gastric mucosal cells to normal physiologic function. The gastroprotective effects of CBS in prevention of gastric lesions induced by various ulcerogenic agents and the mechanism of ulcer healing have been demonstrated in animal studies (Konturek et al., Digestion 37(Supplement 2):8-15, 1987 and Konturek et al., Scandinavian Journal of Gastroenterology 21(Supplement 122):6-10, 1986).

Because of the finding that bismuth is an effective antibacterial agent against H. Pylori, concomitant dosages of bismuth-containing compounds with other anti-ulcer drugs have been increasingly applied in many clinical cases for treatment of peptic ulcers. The most commonly used regiments include double or triple therapy with bismuth; meanwhile, some recent reports regarding quadruple therapy (wherein a proton pump inhibitor is added to triple therapy) have shown eradication rates of over 90%, but also cause severe side effects such as vomiting and diarrhea.

Additionally, while antibacterial therapy (bismuth and amoxycillin or doxycycline) was shown to be effective in eliminating H. Pylori from the gastric mucosa of duodenal ulcer patients, this therapy had no effect on the H. Pylori colonies in their dental plaque (Desai et al., Scandinavian Journal of Gastroenterology 26: 1205-1208, 1991, Nguyen et al., Journal of Clinical Microbiology 31(4):783-787, 1993). The continued presence of H. Pylori in the dental plaque raises the question of whether the relapse of duodenal ulcers is inevitable (Desai et al., Scandinavian Journal of Gastroenterology 26 :1205-1208, 1991 and Abraham et al., Indian Journal of Gastroenterology 9(4):265-6, Editorial, 1990).

Triple therapy, consisting of an antibiotic (amoxicillin, tetracycline or erythromycin), metronidazole, and bismuth compounds, has been reported to result in more than a 95% eradication rate for H. Pylori, and reduced ulcer relapse rate to less than 10% during a 12-month follow-up period (Graham et al., Gastroenterology 102:493-496, 1992 and Borody et al., Gastroenterology 102:A 44, 1992). It is interesting to note that metronidazole as a single agent has only 5% eradication rate for H. Pylori, but as a component of triple therapy, it increases the eradication rate to as high as 95%. When metronidazole-resistant strains of H. Pylori are encountered (about 25% of the H. Pylori strains are resistant), the eradication rate falls to about 50% (Logan et al., Lancet 3:1249-1252, 1991).

One possible explanation for this observed clinical efficacy of metronidazole in combination therapy is that metronidazole is actively secreted in the saliva (Mustofa et al., International Journal of Clinical Pharmacology, Therapy, and Toxicology 29(12):474-478, 1991) where it might be exerting its antimicrobial action against dental plaque-bound H. Pylori colonies. The typical steady state saliva represent 10 to 20 times the MIC for H. Pylori. Another antibiotic, Clarithromycin, a new-generation macrolide, which has shown a 40 to 60% cure rate as a single agent, is also secreted in the saliva. Therefore, it is reasonable to believe that in order to achieve nearly complete eradication of H. Pylori, and prevent peptic ulcer relapse, eradication of this organism from the oral cavity is essential. Colloidal bismuth subcitrate (CBS), the most effective single agent against H. Pylori, is however not absorbed significantly from the GI, and therefore, produces no salivary concentrations. But as a single agent, it is about 6 to 8 times more effective in eradicating H. Pylori than metronidazole. The present invention therefore is related to development of a therapeutic modality to effectively eradicate H. Pylori reservoir from the oral site, as well as the gastric mucosal wall.

The invention relates to concomitant treatment with bismuth compounds and/or with other antibacterial compounds and/or with antibiotics in topical oral and peroral dosage forms to eradicate H. Pylori from its niches both in the dental plaque and in the gastric mucosa in order to improve the ulcer cure rate and prevent ulcer relapse. The invention also provides oral topical dosage forms with pharmaceutically usable bismuth compounds and/or antibacterial compounds and/or antibiotics that eradicate or reduce H. Pylori in dental plaque. The invention further provides for treatment with bismuth compounds and/or antibacterial compounds and/or antibiotics which are effective against Campylobacter rectus and Treponema denticola which are responsible for causing halitosis. The invention also provides bismuth compounds which have applications in wound healing, particularly in ocular and dermal wound healing.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 is a generalized reaction diagram for the synthesis of bismuth sulfates.

FIG. 2 is a graph of human saliva concentration versus time which shows the release of bismuth from CBS chewing gum.

Other novel bismuth-containing compounds which are useful in the present invention are those described in Bos et al., U.S. Pat. No. 4,801,608 and in Serfortein, U.S. Pat. No. 4,153,685, both of which are expressly incorporated herein by reference. Other bismuth compounds, namely complexes of polysulfates, of polyhydroxy compounds such as sugars, sugar alcohols, and ascorbic acid and its derivatives, as well as alpha-D-glucopyranoside bismuth complex, beta-D-fructofuranosyl-oktakis (hydrogen sulfate) bismuth complex, and L-dihydro ascorbyl-tetrakis (hydrogen sulfate) bismuth complex are part of the present invention. A generalized reaction diagram for the synthesis of bismuth sulfates is shown in FIG. 1. These novel compounds will deliver bismuth more effectively and will have less side effects in treating H. Pylori positive gastro duodenal diseases. The compounds will lend themselves to controlled release oral dosage forms and oral topical dosage forms for eradication of H. Pylori in dental plaque.

Chemical structures of the compounds conceived in this invention are complexes of poly-sulfates and of poly-hydroxy compounds such as sugars, sugar alcohols, and ascorbic acid and its derivatives. These novel compounds will deliver bismuth more effectively and will have less side effects in treating H. Pylori positive duodenal ulcers and gastritis. These compounds moreover lend themselves to controlled release oral dosage forms and oral topical dosage forms for eradication of H. Pylori in dental plaque.

Chemical structures of the compounds conceived in this invention are illustrated below:

The ascorbic acid-derived molecules are synthesized in a manner completely analogous to the reaction diagram for synthesis of bismuth sulfates set forth above. These compounds can also be used in embodiments relating to would healing as described below.

In addition to antibacterial bismuth-compounds and antibiotics to the oral cavity for reduction/elimination of Helicobacter pylori in the oral cavity as a means of treatment and prevention of gastrointestinal diseases including peptic ulcers, recurring gastritis, non-ulcer dyspepsia and gastric cancer. Antibiotics useful herein include, but are not limited to, Tetracycline, Amoxicillin, Ampicillin, Doxycycline, Erythromycin, Clarithromycin, Metronidazole, Tinidazole, Ciproflaxacin, Oflaxacin, Norflaxacin, Furazolidine, Nitrofurantoin. Antibacterials useful herein include, but are not limited to naturally occurring peptides and synthetic peptide antibacterials such as Lanthocins, and particularly, Nicin and related peptides, Proton pump inhibitors such as Omeprazole and Lansoprazole, Sanguinaria and other antibacterials obtained from plant sources, as well as bismuth-containing compounds.

Each oral-topical dosage form of this invention is the one which can make it possible to release bismuth compound and/or antibacterial compounds and/or antibiotics into oral cavity in a predictable manner and result in appropriate antibacterial concentration. Those examples of such forms include a chewing-gum form, a chewable form including chewable tablets, lozenges, dental paints, viscous gels, dental implants, polymer film adhesives, a troche form, a toothpaste form, a gargling-gel form and mouth-rinse form. Preferably, a chewing-gum form and a troche form are chosen. Further, a chewing-gum form is most preferred due to its easy-to-use characteristic, predictable drug release and increased drug contact with dental surface. The chewing gum delivery system specially enables sustained contact of the antibacterial agents with the entire oral cavity and therefore, enhance bactericidal/bacteriostatic efficacy. We have already demonstrated that chewing gum formulation containing an antibacterial agent, colloidal bismuth subcitrate, releases the drug in a precise and reproducible fashion during a 15 minute chewing time. Chewable tablets, viscous gel formulations, and dental paint formulations also will be able to provide sustained concentration of antibacterial agents in the oral cavity.

Oral-topical dosage forms containing bismuth in this invention must release enough bismuth, antibiotic, and/or antibacterial into saliva for eradication of H. Pylori in the oral cavity. The minimum inhibitory concentration (MIC) of bismuth for H. Pylori varies in each bismuth compound. For instance, it is reported that the MIC of CBS for H. Pylori is 8 mg/L and its range is 4 to 32 mg/L.

Therefore, the dosage form should release bismuth into saliva up to at least two times the MIC, preferably a minimum of 2 to 10 times, most preferably 2 to 250 times. In order to achieve this level of release rate, the bismuth content per dosage form should be about 50 mg to 200 mg, preferably a minimum of 10 mg to 50 mg, most preferably 25 mg to 50 mg. For instance, each piece of CBS-containing chewing gum should contain approximately 50 mg to 200 mg of CBS, preferably a minimum of 10 mg to 50 mg, most preferably 25 mg to 50 mg.

Time release of each dosage form in this invention must be long enough to eradicate H. Pylori. Although the duration of time release varies in each bismuth compound and in each dosage form, it is desirable that at least 25% of the dose is released within 2 minutes, more preferably at least 35%, more preferably at least 45%, more preferably at least 55%, more preferably at least 65%, most preferably at least 75%, more preferably within 2 to 15 minutes, most preferably within 10 to 15 minutes.

In other preferred embodiments of the invention presented herein, a chewing gum drug delivery system is utilized to provide sustained concentration of bismuth compounds, antibiotics, and/or antibacterial compounds which are proven antibacterial agents against H. Pylori and anti-plaque agents to help these compounds penetrate the dental plaques to reach the site of H. Pylori infection. The chewing gum delivery system enables sustained contact of the antibacterial agents with the entire oral cavity and therefore, enhances bacteriocidal efficacy.

Where antibiotic and/or antibacterial agents other than bismuth are to be used, oral-topical dosage form in this invention must release enough antibiotic/antibacterial into saliva for eradication of H. Pylori from the oral cavity. The minimum inhibitory concentration (MIC) varies for each antibiotic/antibacterial agent. However, for most of the antibiotics listed in this invention, the MIC values are between less than 1 to 10 mcg/mL, or 1 to 10 mg/L.

Therefore, the topical-oral dosage from should release the anti-bacterial agent into saliva up to at least 2 times the MIC, preferably a minimum of 2 to 10 times, most preferably 2 to 100 times. In order to achieve this level of release, the antibacterial content per unit of dosage form should be about 10 to 100 mg, preferably a minimum of 5 to 50 mg, most preferably 10 to 25 mg. For instance, each piece of chewing gum should contain approximately 10 to 100 mg. of the antibiotic or antibacterial agent. Preferably a minimum of 5 to 50 mg, most preferably 10 to 25 mg.

The topical-oral dosage forms of this invention must release the antibiotic/antibacterial over an extended time. The duration of release should be at least 5 minutes, preferably 10 minutes, most preferably 15 minutes. Further, at least 25% of the dose is released within 5 minutes, more preferably at least 35%, more preferably at least 45%, more preferably at least 55%, more preferably at least 65%, most preferably at least 75% of the antibiotics/antibacterial content should be released within 5 minutes, preferably within 2 to 15 minutes, most preferably within 10 to 15 minutes.

In other preferred embodiment of this invention, a chewing gum delivery system is utilized to provide sustained concentration of antibiotic/antibacterial agent several times above its MIC for H. Pylori over at least 10 times.

The anti-plaque agents further contribute to improved efficacy by breaking down the plaque and exposing the bacterial colonies to the antibacterial agents. The chewing gum formulation containing CBS, antibiotic, and/or antibacterial releases the drug in a precise and reproducible fashion during a 15-minute chewing time. Anti-plaque agents include, but are not limited to, glucanase anhydroglucosidase, glucose oxidase, silicon oil, sanguinarine, and the like. Chewing gum formulations may optionally include crystalline sorbitol, sorbitol solution, mannitol, Nova-base™, or any other gum base, dextrans, cellulose derivatives, buffer salts, sweeteners, flavors, and the like.

Optionally, metronidazole can be added to CBS chewing gum to broaden the antimicrobial activity against H. Pylori.

Bismuth compounds embodied in these inventions also have been found to stimulate cellular production of growth factors, and therefore have applications in wound healing, specifically in ocular and dermal wound healing. Therefore, the present invention also contemplates use of novel bismuth complexes with sulfated polyhydroxy hydrophilic film-forming polymers to accelerate wound healing in ulcerative diseases of the eye, skin, and other mucosal tissues. For these embodiments, the invention involves synthesis of unique complexes of bismuth with partially sulfated hydrophilic film-forming polymers such as hydroxyprobyl cellulose, hydroxyethyl cellulose, hydroxypropyl-methyl cellulose, carboxymethyl cellulose, and polyvinyl alcohol. These compounds are formulated in unique film-forming solutions, aerosols, and gels for treatment of corneal ulcers, skin ulcers, gastric ulcers, and other wounds of the skin and mucous membranes. The general structures of this class of complexes are represented below:

EXAMPLE 1Preparation of Therapeutic Substance

To an aqueous solution of ammonia are added bismuth citrate, citric acid, and caustic potash in specific stoichiometric proportions, and at specific temperatures. The solution is examined for turbidity and, if required, additional volume of ammonia solution is added to render the solution clear. The solution is then filtered on a carbon bed and spray dried to obtain free-flowing powder material. The product is packaged in an air and moisture proof glass container.

EXAMPLE 2Preparation of Topical Dosage Form

Brief general description of the preferred topical dosage form, chewing gum, is set forth as follows. Fully melt the gum base (at approximately 90° C.) in Brabender mixer, a jacketed mixer with sigma blades. Remove the hot water from the mixer jacket, allow to cool, and add lecithin and mix well. Cool further to approximately 50° C., and add liquid flavor and mannitol. Mix until uniform. Dry blend colloidal bismuth subcitrate in sorbitol, and blend sodium citrate in sorbo syrup. Add sorbitol and sorbo syrup blends to the gum base. Cool the product to 35° C., add flavor and sweetener and mix until smooth. Remove the product from the mixing kettle, roll to form a sheet of uniform thickness and score to produce chewing gum sticks weighing 2.5 g each. Wrap individual gum sticks in aluminum foil and place in plastic bags. Where the gum is to include antibiotic or antibacterial compounds, the agent is coated with a polymeric substance to mask any untoward taste or odor, and to further regulate its release in the saliva.

EXAMPLE 3Composition of CBS-Containing Gum

Two variations of the 50 mg CBS gum (Table 1) were used. Both formulations used were identical with the exception that Formula-2 contained sodium citrate to impart a firmer texture, while Formula-1 did not.

Moderately water soluble bismuth compounds such as bismuth ascorbyl sulfate, bismuth sucrose sulfate, bismuth subascorbate, cyclodextrin bismuth sulfate are used in the chewing gum dosage form to produce sustained concentration in the saliva.

Synthetic and natural latex-based chewing gum bases are used to tightly enclose bismuth compounds and other antibacterial/antibiotic compounds to cause their gradual release in the saliva.

These formulation/composition modifications are designed to:

(1) provide control release of antibacterial/antibiotic compounds to increase their bactericidal efficacy against oral cavity/dental plaque bound H. Pylori; and

Among six healthy human subjects, who gave informed consent, three chewed the CBS-containing gum with sodium citrate, and the other three chewed CBS-containing gum without sodium citrate. The subjects chewed the gum samples for a total of 15 minutes. Saliva samples were collected at time interval of 0, 1, 5, 10, and 15 minutes of chewing. The saliva samples were then submitted to an analytical laboratory for bismuth analysis. Results are shown in Table 2.

TABLE 2

IN VIVO SALIVARY CONCENTRATION OF

CBS FROM THE CHEWING GUM

chewing

time

saliva

conc of Bi

conc of active

Formula

(min.)

vol. (mL)

(ppm)

CBS (u/mL)

X MIC

formula-1

0

4.4

(± 0.5)

1

3.3

(± 1.4)

900.7

(± 239.1)

1270.3

(± 334.7)

148.7

(± 42.0)

5

5.4

(± 1.5

247.7

(± 112.3)

363.3

(± 158.9)

45.0

(± 19.9)

10

4.9

(± 1.3)

28.0

(± 5.0

40.0

(± 6.6)

5.0

(± 1.0)

15

5.2

(± 2.1)

15.8

(± 17.8)

25.7

(± 23.0)

3.1

(± 2.7)

formula-2

0

7.2

(± 0.5)

1

4.8

(± 1.9)

888.3

(± 329.5)

1257.0

(± 464.5)

156.3

(± 58.0)

5

8.5

(± 1.7)

326.0

(± 113.3)

572.7

(± 159.7)

63.7

(± 19.9)

10

7.5

(± 3.4)

30.0

(± 9.5)

42.3

(± 13.6)

5.0

(± 1.7)

15

7.7

(± 3.8)

10.7

(± 6.7)

14.7

(± 9.2)

1.8

(± 1.2)

Saliva samples were analyzed for elemental bismuth in ppm units. The results were then converted to mg of active CBS per mL of saliva and also expressed as a multiple of minimum inhibitory concentration (MIC) of CBS for H. Pylori. As can be seen from the results (formula-2 of Table-3), the salivary concentrations of CBS are 156, 64, 5, and 1.8 times the MIC at 1, 5, 10 and 15 minutes, respectively. The constant bathing of the oral cavity from saliva containing sufficient concentration of CBS (2 to 5 times the MIC) for up to 15 minutes can be expected to further reduce the viable cells of H. Pylori. These results are plotted in FIG. 2 which a graph of human saliva concentration versus time.

EXAMPLE 5Sensory Analysis of Chewing Gum

Sensory characteristics of the chewing gum were evaluated by the subjects during the 15 minutes of chewing. Again, three subjects chewed the CBS gum containing sodium citrate and three subjects chewed the CBS gum without sodium citrate. A nine point rating scale was used to evaluate each category (Tables 3 and 4).

TABLE 3

RESULTS OF SENSORY ANALYSIS RATING OF CBS GUM

WITHOUT SODIUM CITRATE

(Formula-1)

SENSORY

CHEWING TIME

CHARACTERISTICS

1 MIN

5 MIN

10 MIN

15 MIN

Overall Flavor

6.3

6.0

5.3

5.0

(0 = dislike extremely,

(± 1.2)

(± 1.0)

(± 1.5)

(± 1.0)

8 = like extremely)

Flavor Intensity

5.7

4.7

3.7

3.0

(0 = none, 8 = very strong)

(± 1.5)

(± 1.2)

(± 0.6)

(± 1.0)

Chew Qualities

6.0

6.0

5.3

5.0

(0 = dislike extremely,

(± 1.0)

(± 1.0)

(± 1.5)

(± 1.0)

8 = like extremely)

Unpleasant Aftertaste

0.0

0.0

0.0

0.0

(0 = none, 8 = very strong)

(± 0.0)

(± 0.0)

(± 0.0)

(± 0.0)

Overall Qualities

6.3

6.0

5.7

5.3

(0 = dislike extremely,

(± 1.2)

(± 1.0)

(± 1.2)

(± 1.5)

8 = like extremely)

TABLE 4

RESULTS OF SENSORY ANALYSIS RATING OF CBS GUM

WITHOUT SODIUM CITRATE

(Formula-2)

SENSORY

CHEWING TIME

CHARACTERISTICS

1 MIN

5 MIN

10 MIN

15 MIN

Overall Flavor

6.7

5.7

4.7

4.7

(0 = dislike extremely,

(± 0.6)

(± 1.5)

(± 1.2)

(± 1.2)

8 = like extremely)

Flavor Intensity

6.7

6.0

5.0

3.7

(0 = none, 8 = very strong)

(± 0.6)

(± 0.0)

(± 1.0)

(± 1.5)

Chew Qualities

4.7

5.0

4.3

4.3

(0 = dislike extremely,

(± 2.1)

(± 2.0)

(± 1.5)

(± 0.6)

8 = like extremely)

Unpleasant Aftertaste

0.7

1.7

1.7

2.0

(0 = none, 8 = very strong)

(± 1.2)

(± 2.1)

(± 2.1)

(± 2.0)

Overall Qualities

6.3

5.7

4.7

4.0

(0 = dislike extremely,

(± 0.6)

(± 1.2)

(± 1.2)

(± 1.0)

8 = like extremely)

In general, there were no dramatic differences in the sensory analysis between the two formulas. The sensory panel clearly shows that both chewing gum formulations have a desirable level of flavor and taste, and cause a ninimal unpleasant aftertaste after chewing.

EXAMPLE 6Topical Safety

Topical safety was evaluated in the six volunteers for up to 60 minutes after administration of the gum. The subjects were asked to report any adverse effects such as discomfort or irritation in the oral cavity.

There were no reports of any discomfort or irritation in the oral cavity by any of the subjects at either the 15 or 60 minute post administration time periods.

EXAMPLE 7Storage Stability Study

Samples of CBS-containing gum (50 mg) were wrapped individually in foil wrappers. The sticks of gum were then placed in foil laminate bags, sealed, and placed in storage. Storage conditions include 40° C. and room temperature (RT). The duration of the stability testing was 90 days. The results are shown in Tables 5-8 below.

Each stick of the gums used for the stability study (1 for zero-time, 2 for three month, total 3 sticks) was from the same lot number. The results show that bismuth concentration remains stable over the tested time period.

EXAMPLE 8Denture Material Exposure Study

An evaluation of CBS salivary concentration on various denture materials was conducted in order to test any potential staining effect of the CBS on denture materials. Artificial saliva was used (Table 9).

TABLE 9

THE COMPOSITION OF ARTIFICIAL SALIVA

Concentration

Ingredients

per Liter

Sodium Bicarbonate

0.50 g

Sodium Phosphate, Dibasic, Dihydrate

0.85 g

Calcium Chloride

0.44 g

Magnesium Chloride

0.06 g

Potassium Chloride

1.40 g

Sodium Carboxyl Methyl Cellulose

2.00 g

Phosphoric Acid to adjust pH to 6.4 Distilled Water

QS

The test saliva was prepared by dissolving 0.500 g of colloidal bismuth subcitrate in 100 mL of the above artificial saliva. 500 mL of Artificial Saliva (RT) was placed in one of two identical glass jars with lids. In the other jar was placed 500 mL of the Artificial Saliva (RT) containing 0.50% of CBS. In each of the jars the denture material block and a magnetic stirrer was placed. The jars were then placed on the magnetic platform and set to agitate at a minimum rate. The denture materials that were exposed to artificial saliva containing CBS or placebo included (Table 10).

TABLE 10

DENTURE MATERIALS

1) Natural tooth with silver amalgam filling

2) Composite resin (used on anterior teeth for filling)

3) Denture base acrylic resin

4) Porcelain fused to metal

5) Partial denture metal frame

6) Acrylic tooth (artificial)

7) Natural tooth

The four hour exposure of natural tooth and other denture materials to 0.5% CBS in artificial saliva with mild agitation did not cause any staining, discoloration, or changes in texture.

EXAMPLE 9Clinical Efficacy Data

An open label, placebo-controlled pilot clinical study in ten patients with initial positive response for H. Pylori in the dental plaque has been initiated. Data from six patients (four patients treated with CBS 50 mg chewing gum six times-a-day and two patients treated with placebo chewing gum six times-a-day for fifteen days) has been obtained. The dental plaque samples from the patients were collected before treatment, day 7 and day 15 after treatment, and tested by microbiological culture and CLO test. The results are set forth in Table 11 below:

TABLE 11

SIDE

DUR POSITIVE

EFFECTS

CLO

(HRS:MINS)

CULTURE

(Stain/Odor)

TREATED GROUP (n = 4)

Pt 1

Day 0

+

1:00

+

NE

30/M

Day 7

+

1:45

−ve

—

Day 15

+

1:30

−ve

—

Pt 2

Day 0

+

2:15

+

NE

42/M

Day 7

+

1:30

NA

—

Day 15

+

4:00

−ve

—

Pt 3

Day 0

+

2:30

+

NIL

31/M

Day 7

+

4:30

NA

NIL

Day 15

+

5:30

NA

NIL

Pt 4

Day 0

+

2:30

NA

NIL

29/F

Day 7

+

4:00

NA

NIL

Day 15

+

5:30

NA

NIL

Mean CLO response time after 15 days = 4.125 HR

PLACEBO (n = 2)

Pt 1

Day 0

+

1:00

NA

NIL

26/M

Day 7

+

1:30

NA

NIL

Day 15

+

1:30

NA

NIL

Pt 2

Day 0

+

1:15

NA

NIL

28/M

Day 7

+

2:00

NA

NIL

Day 15

2:30

NA

NIL

Mean CLO response time after 15 days = 2.0 HR

NA = Not available

NE = Not evaluated (before chewing)

The data show that for patients treated with CBS 50 mg chewing gum and placebo chewing gum on day 15 the mean CLO response times are 4.125 hours and 2.0 hours, respectively. The longer CLO test response time for CBS 50 mg chewing gum group compared to the placebo chewing gum group is indicative of substantial reduction in H. Pylori density in the oral cavity of the active treatment group.

EXAMPLE 10Toxicology

A number of animal toxicity studies and human clinical investigations have demonstrated safety of bismuth compounds, especially CBS, in therapeutic dose ranges. No toxicity has been reported in chronic daily administration of high doses of CBS (160, 320, and 640 mg/kg body weight representing 2, 4, and 8 times the human therapeutic dose respectively) in rats treated for three months or dogs treated for six months. See Wieriks et al., Journal of Gastroenterology 17(Supplement 80):11-16 (1982), incorporated herein by reference.

Long term safety of CBS and treatment of peptic ulcers at a standard dose of 480 mg (expressed as bismuthtrioxide) in four daily divided doses has been examined by Bader, Digestion 37(Supplement 2):53-59 (1987), incorporated herein by reference. CBS was first introduced in Europe in 1971 and since that time 1.5 million treatments have been dispensed. During eight years of use of CBS tablets [De-Nol(R)®] in Europe between 1978 and 1986 under a more comprehensive adverse reaction monitoring system, only 13 adverse reaction forms were completed. Five of these adverse reactions were ascribed to CBS: one case of headache, one case of stomach pain, one case of diarrhea, and two cases of allergy (mainly in the form of skin rashes). A high degree of safety of CBS in therapeutic applications for the treatment of peptic ulcers is reported in a recent review of pharmacology of bismuth-containing compounds by Lambert, Review of Infectious Diseases 13(Supplement 8):691-695 (1991), incorporated herein by reference. In reviewing safety and pharmacokinetics of CBS, Bennet, Scandinavian Journal of Gastroenterology 26(Supplement 185):29-35 (1991), incorporated herein by reference, has calculated the systemic bioavailability of bismuth after oral dosing of CBS to be in the range of 0.16 to 0.28% of the administered dose, and concluded that steady-state blood levels of 50-100 mg/mL are unlikely to cause any neurotoxicity.

Saliva samples are analyzed for antibiotic or antibacterial agents in ppm units. The results are then converted to mg of active agent per mL of saliva and also expressed as a multiple of minimum inhibitory concentration (MIC) of the agent for H. Pylori. The salivary concentrations of the agent are 156, 64, 5, and 1.8 times the MIC at 1, 5, 10 and 15 minutes, respectively. The constant bathing of the oral cavity from saliva containing sufficient concentration of the agent (2 to 5 times the MIC) for up to 15 minutes can be expected to further reduce the viable cells of H. Pylori; These results are plotted to show a graph of human saliva concentration versus time.

Sensory characteristics of the chewing gum are evaluated by the subjects during the 15 minutes of chewing. Again, three subjects chews the gum containing sodium citrate and three subjects chewed the gum without sodium citrate. A nine point rating scale is used to evaluate each category.

In general, there are no dramatic differences in the sensory analysis between the two formulas. The sensory panel shows that both chewing gum formulations have a desirable level of flavor and taste, and cause a minimal unpleasant aftertaste after chewing.

Topical safety is evaluated in the six volunteers for up to 60 minutes after administration of the gum. The subjects are asked to report any adverse effects such as discomfort or irritation in the oral cavity.

There are no reports of any discomfort or irritation in the oral cavity by any of the subjects at either the 15 or 60 minute post administration time periods.

Samples of the agent-containing gum (5mg) are wrapped individually in foil wrappers. The sticks of gum are then placed in foil laminate bags, sealed, and placed in storage. Storage conditions include 40° C. and room temperature (RT). The duration of the stability testing is 90 days.

Each stick of the gums used for the stability study (1 for zero-time, 2 for three month, total 3 sticks) is from the same lot number. The results show that bismuth concentration remains stable over the tested time period.

An evaluation of salivary concentration of the agent on various denture materials is conducted in order to test any potential staining effect of the CBS on denture materials. Artificial saliva is used (Table 9).

The test saliva is prepared by dissolving 0.500 g of the antibiotic or antibacterial agent in 100 mL of the above artificial saliva. 500 mL of Artificial Saliva (RT) is placed in one of two identical glass jars with lids. In the other jar is placed 500 mL of the Artificial Saliva (RT) containing 0.50% of the agent. In each of the jars the denture material block and a magnetic stirrer is placed. The jars are then placed on the magnetic platform and set to agitate at a minimum rate. The denture materials that are were exposed to artificial saliva containing the agent or placebo are included. The four hour exposure of natural tooth and other denture materials to 0.5% of the agent in artificial saliva with mild agitation does not cause any staining, discoloration, or changes in texture.

To assess clinical efficacy, patients with positive response for the presence of H. Pylori in the dental plaque/oral cavity are divided into two treatment groups. Group I is given placebo chewing gum to be chewed 2 or 6 times a day for 2 or 4 weeks. Group II is given chewing gum containing antibiotic/antibacterial agent to be chewed 2 or 6 times a day for 2 or 4 weeks. Patient's dental plaque/saliva samples are collected at time 0 (Pre-treatment) on days 7, 14, 28, and tested for H. Pylori presence and density. The incidence of H. Pylori presence in the placebo group and the active treatment group is compared. The group receiving the chewing gum containing antibiotic/antibacterial shows significantly lower incidence of H. Pylori presence in the dental plaque/saliva compared to placebo chewing gum group after 2 and 4 weeks of treatment.

EXAMPLE 12Antibacterial Efficacy for Treatment of Halitosis

Campylobacter rectus, Helicobacter pylori, and Treponema denticola have been demonstrated to be associated with Halitosis (bad breath). The compounds and methods of the present invention, including CBS as well as ascorbyl bismuth derivative, have demonstrated in vitro activity against all three bacteria, as indicated by their minimum effective concentrations (MICs) presented in Table 12 below.

TABLE 12

Bismuth

Bismuth

Ascorbyl Sulfate

Sucrose Sulfate

CBS

Test Organisms

(μg/mL)

(μg/mL)

(μg/mL)

Campylobacter rectus

256

>256

256

Helicobacter pylori

8

16

2

Treponema denticola

16

32

32

EXAMPLE 13In Vitro Mesentery Culture Model

Colloidal bismuth subcitrate and other bismuth compounds are known to accelerate wound healing by increasing the concentration of epithelial growth factor (EGF) and fibroblast growth factor (FGF) in the wounded tissue.

Utilizing a rat mesentery culture model (Wu et al., Annals of Plastic Surgery 33(2):155-161 (1994), incorporated herein by reference) and a medium containing 2% fetal calf serum, wound closure rates are measured. This tissue culture model is useful for gaining insights into growth factor interactions and wound healing. CBS or bismuth ascorbyl sulfate or glucose (placebo) are added to the medium in concentration ranges from 10 mcg/mL to 1,000 mcg/mL, and the wound closure is assessed at 24-hour, 48-hour and 72-hour intervals. Significantly higher concentrations of growth factors EGF and FGF are observed. Moreover, a significantly faster wound closure rate and complete closure is seen in the culture to which CBS or bismuth ascorbyl sulfate are added, compared to the placebo.

The efficacy of CBS and bismuth ascorbyl sulfate at enhancing wound healing is also studied in a freeze-injured skin graft model for quantitative evaluation of promoters of wound healing (Lees et al., British Journal of Plastic Surgery 47(5):349-359 (1994), incorporated herein by reference). Application of CBS or bismuth ascorbyl sulfate stimulates wound healing in cryoinjured grafts in a dose-related fashion. Doses of 10 to 1000 mcg/mL produce significant increase in wound healing rates compared to placebo.

Topical dosage forms for wound healing will depend on whether corneal or dermal wound healing is sought. For dermal wound healing, occlusive or non-occlusive barriers can be used to achieve a pharmacologically desirable concentration over a desirable duration (i.e., sustained release). For corneal wound healing, it is desirable to release the dosage of bismuth compound over a period of at least 30 minutes, more preferably at least 1 hour, more preferably at least 6 hours, more preferably at least 12 hours, more preferably at least 24 hours, more preferably at least 36 hours, more preferably at least 48 hours, more preferably at least 60 hours, more preferably at least 72 hours. For both dermal and corneal treatment, the release of bismuth compounds should provide a concentration of at least 10 μg/mL, more preferably at least 100 μg/mL, more preferably at least 500 μg/mL, more preferably at least 1 mg/mL, more preferably at least 10 mg/mL, more preferably at least 100 mg/mL.

Dermal wound healing as disclosed herein also contemplates the treatment of acne vulgaris to eliminate bacteria and to repair epithelial cell damage. For this use, the topical dosage form should be able to penetrate the acne comedone (i.e., pustule having crusty surface), should permit comfortable application, and should not cause irritation of acne. As disclosed herein, suitable dosage forms include creams, gels, ointments, suspensions, etc., and will provide therapeutic concentrations as set forth above.

Thus, while several embodiments have been shown and described, various modifications may be made, without departing from the spirit and scope of the present invention.